Peptide Based Inhibitors of Protein Binding to the Mitogen-Activated Protein Kinase Docking Groove

被引:9
|
作者
Alexa, Anita [1 ]
Ember, Orsolya [1 ,2 ]
Szabo, Ildiko [3 ]
Mo'ath, Yousef [2 ]
Poti, Adam L. [1 ]
Remenyi, Attila [1 ]
Banoczi, Zoltan [2 ]
机构
[1] Inst Organ Chem, Res Ctr Nat Sci, Biomol Interact Lab, Budapest, Hungary
[2] Eotvos Lorand Univ, Inst Chem, Dept Organ Chem, Budapest, Hungary
[3] Eotvos L Univ, MTA ELTE Res Grp Peptide Chem, Eotvos Lorand Res Network ELKH, Budapest, Hungary
关键词
mitogen-activated protein kinase; protein-protein interaction; peptide inhibitor; cellular uptake; cell-penetrating peptide; MACROCYCLIC PEPTIDES; IN-VIVO; DISCOVERY; CARRIERS; CELLS; MAPKS;
D O I
10.3389/fmolb.2021.690429
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Mitogen-activated protein kinases (MAPK) are important regulatory units in cells and they take part in the regulation of many cellular functions such as cell division, differentiation or apoptosis. All MAPKs have a shallow docking groove that interacts with linear binding motifs of their substrate proteins and their regulatory proteins such as kinases, phosphatases, scaffolds. Inhibition of these protein-protein interactions may reduce or abolish the activity of the targeted kinase. Based on the wide range of their biological activity, this kind of inhibition can be useful in the treatment of many disorders like tumors, inflammation or undesired cell apoptosis. In this study a linear binding motif from the RHDF1 protein-a 15 amino acids long peptide-was selected for optimization to increase its cellular uptake but retaining its low micromolar binding affinity. First, we synthesized an octaarginine conjugate that showed efficient cellular uptake. Next, we set out to reduce the size of this construct. We were able to decrease the length of the original peptide, and to increase its cellular uptake with specific chemical modifications. These new constructs bound better to ERK2 and p38 kinases than the original peptide and they showed markedly increased cellular uptake. The new octaarginine conjugate and one of the minimized bicyclic derivatives could inhibit the phosphorylation of intracellular ERK or p38. However, the modulation of MAPK phosphorylation levels by these cell-penetrating peptides were complex, despite that in biochemical assays they all inhibited MAPK-substrate binding as well as phosphorylation. The optimized peptides depending on the applied concentration caused an expected decrease, but also some unexpected increase in MAPK phosphorylation patterns in the cell. This possibly reflects the complexity of MAPK docking groove mediated protein-protein interactions including bone fide MAPK clients such activator kinases, deactivating phosphatases or regulatory scaffolds. Thus, our findings with optimized cell-penetrating "inhibitory" peptides highlight the opportunities but also the pitfalls of docking peptide based MAPK activity regulation and call for a better quantitative understanding of MAPK mediated protein-protein interactions in cells.
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页数:11
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